Impact of Sprouting under Potassium Nitrate Priming on Nitrogen Assimilation and Bioactivity of Three Medicago Species

Edible sprouts are rich in flavonoids and other polyphenols, as well as proteins, minerals, and vitamins. Increasing sprout consumption necessitates improving their quality, palatability, and bioactivity. The purpose of this study was to test how KNO3 priming affects the sprouting process species on three Medicago species (Medicago indicus, Medicago interexta, and Medicago polymorpha) and their nutritional values. Targeted species of Medicago were primed with KNO3, and the levels of different primary and secondary metabolites were determined. KNO3 induced biomass accumulation in the sprouts of the three species, accompanied by an increased content of total mineral nutrients, pigments, vitamins, and essential amino acids. Besides, our results showed that KNO3 enhanced the activity of nitrate reductase (NR), glutamate dehydrogenase (GDH), and glutamine synthetase (GS) enzymes, which are involved in the nitrogen metabolism and GOGAT cycle, which, in turn, increase the nitrogen and protein production. KNO3 treatment improved the bioactive compound activities of Medicago sprouts by increasing total phenolic and flavonoid contents and enhancing the antioxidant and antidiabetic activities. Furthermore, species-specific responses toward KNO3 priming were noticeable, where Medicago interexta showed the highest antioxidant and antidiabetic activities, followed by Medicago polymorpha. Overall, this study sheds the light on the physiological and biochemical bases of growth, metabolism, and tissue quality improvement impact of KNO3 on Medicago sprouts.


Introduction
One of the natural processing methods for increasing the nutritional value and health qualities of foods is the sprouting of seeds. This approach has been employed in Eastern countries for a long time [1]. Since the sprouts are eaten so early in their growth cycle, their nutrient content remains very high [2]. Sprouts are excellent sources of protein, vitamins, and minerals, as well as essential nutrients for promoting health, such as glucosinolates during the sprouting process are not quite understood. Therefore, the purpose of this study was to assess the impact of KNO 3 priming on growth, N metabolism, tissue quality, and biological values in the sprouts of three species of Medicago.

Plant Material and Growth Conditions
Seeds of Medicago (Medicago indicus, Medicago interexta, and Medicago polymorpha) were collected from the Agricultural Research Center (Giza, Egypt), where they were collected during filed trips to different locations in Egypt (Giza and Ismailia). Before being stored in distilled water overnight, the seeds were rinsed in distilled water and submerged in 5 g L −1 sodium hypochlorite for 1 h. Two hundred seeds were clustered into a group soaked in distilled water (control), and the second group was soaked in a KNO 3 solution of 25 mM, for 16 h. The applied growth promoting concentration of KNO 3 was selected according to a pilot experiment, where five concentrations (0 and 10, 15, 25, 50 mM) were tested. Each species seeds were evenly placed on 10 vermiculite-lined trays, which were irrigated every two days with Milli-Q water, and each tray received 150 mL of aquaponic water. The experiment was conducted in a growth cabinet under controlled conditions (25 • C, 16 h light/8 h dark cycle, and PAR of 400 µmol m −2 s −1 and relative humidity of 60% per day). After ten days, the fresh mass of each sprout was measured and then stored at −80 • C for further biochemical analyses. Experiments were repeated 4 times, and 20 plants that were pooled from each tray and treated (biological replicate) were used for each measurement.

Analysis of Mineral Contents
Two hundred milligrams of each KNO 3 -primed Medicago sprout was processed in an oven with an HNO 3 /H 2 O solution (5:1 v/v) to determine macro and micro-elements. The concentrations of macro-minerals and trace elements at 25 • C were measured using inductively coupled plasma mass spectrometry (ICP-MS, Finnigan Element XR, and Scientific, Bremen, Germany), with nitric acid in one percent employed as standards [19]. Tandard solution of multielement was used for calibration solution preparation at concentrations form 0 to 50 ppm in 2% HNO 3 . Nitric acid was used as blank. Medicago sprout samples were vaporized, atomized, and ionized inside the chamber of the plasma. The limits of detection (LODs) and quantification (LOQs) values ranged from 0.0002 to 0.01 ug kg −1 and 0.004 to 0.3 µg kg −1 , respectively.

Determination of Leaf Pigments
The frozen Medicago sprout samples (0.5 g) were homogenized in acetone for 1 min at 7000 rpm using a MagNALyser (Roche, Vilvoorde, Belgium), and then centrifuged for 20 min at 14,000× g at 4 • C [20]. Acrodisc GHP filter (0.45 µm/13 mm) was used to filter the supernatant. The solution was then evaluated by HPLC (Shimadzu, SPDM10Avp, Japan, Tokyo) at reversed-phase and at 4 • C [19]. Pigment and carotenoid separation was carried out on a silica-based C18 column (Waters, Spherisorb, 5 m ODS1, 4.6 250 mm) with two different solvents: (A) acetonitrile: methanol: water in the ratio of 81:9:10, and (B) methanol: ethyl acetate in the ratio of 68:32. A diode-array detector (Shimadzu SPDM10Avp) was used to analyze the extraction of chlorophyll a and b, beta-carotene, and xanthophylls at four distinct wavelengths (420, 440, 462, and 660 nm), respectively.

Determination of Amino Acids
Medicago sprouts (300 mg fresh weight (FW)) samples were extracted in methanol [19]. GC/MS (Hewlett Packard, Palo Alto, CA, USA) analysis was carried out, and samples were separated on a HP-5 MS column. Two hundred milligrams of FW sprout leaves were homogenized in 80% aqueous ethanol and centrifuged at 22,000× g for 25 min to measure the amino acids. The supernatant was evaporated, and the precipitates were resuspended in chloroform. The pellet was re-dissolved in chloroform and was filtered (0.2-µm Millipore microfilters). Amino acids levels were measured by Waters Acquity UPLC-tqd system at 37 • C, low pressure, and mobile phase acetonitrile/water ration 60/40, with a measurement at 254 nm. The result was expressed in mg/g dry weight of the sample.

Determination of Polyphenols and Flavonoid Contents
One hundred milligrams of frozen sprouts were homogenized in 1 mL of 80% ethanol (v/v) to extract polyphenols and flavonoids [21]. The supernatant was utilized to determine the total phenolic and flavonoid contents after centrifugation at 4 • C for 20 min. A Folin-Ciocalteu test, with gallic acid as a standard, was used to assess phenolic content. The modified aluminum chloride colorimetric method was used to quantify flavonoid concentration, utilizing quercetin as a standard [22].

Determination of Vitamin Contents
Using UV and/or fluorescence detectors, the amounts of ascorbate, tocopherols, thiamine, and riboflavin in sprouts were measured [19]. For thiamine, and riboflavin extraction, 250 mg of sample were extracted in 0.1 N HCl for 30 min [23]. Samples were separate through a 5 µm C18 Luna Phenomenex stainless steel column (250 × 4.6 mm i.d.). The mobile phase (methanol:sodium acetate (40:60 v/v) was used, and the fluorometric detection was performed at 453 nm and 580 nm, for riboflavin, and 366 nm and 453 nm, for thiamine. At 4 • C, ascorbate (vitamin C) was extracted in 1 mL of 6% (w/v) meta-phosphoric acid and separated using reversed-phase HPLC with a UV detector (100 mm 4.6 mm Polaris C18-A, 3 lm particle size; 40 • C, isocratic flow rate: 1 mL min1, elution buffer: 2 mM KCl, pH 2.5 with O-phosphoric acid). Tocopherol (vitamin E) was separated on a Particil Pac 5 m column (length 250 mm, i.d. 4.6 mm) and measured using HPLC (Shimadzu's Hertogenbosch, normal phase conditions) and a fluorometric detector (excitation at 290 nm and emission at 330 nm). On a reverse-phase (C18) column, riboflavin and thiamine were separated (HPLC, methanol:water as mobile phase, and fluorescence as a detector).

Determination of Total Proteins
The protein was measured according to the Folin-Lowry. Two-tenths of a gram of frozen Medicago sprouts were homogenized in chloroform/methanol (2:1, v/v) solution and centrifuged for 15 min at 3000× g to measure the total proteins content [24].

Determination of N, Ammonium, and Nitrate Contents
The amount of nitrate in the water was determined using Cataldo et al.'s method [25]. Here, 0.1 mL filtrate and 0.4 mL 5% salicylic acid in concentrated H 2 SO 4 made up the reaction mixture. After cooling at ambient temperature for 15 min, 9.5 mL 2 M NaOH was progressively added to elevate the pH above 12. The absorbance was measured at 410 nm when the solution was cooled to room temperature. Nitrate concentration was determined using a KNO 3 calibration curve and represented in mg NO 3 -g −1 FW. The amount of ammonium in the sample was determined using the indophenol blue colorimetry method at 630 nm. The standard was ammonium chloride. Total N was measured using fine ground leaf dry samples (0.2 g) digested with H 2 SO 4 -H 2 O 2 at 260 • C.
2.9. Determination of Antioxidant and Antidiabetic Activities 2.9.1. Antioxidant Activity Each Medicago sprout sample (0.1 g) was extracted in 80 percent ethanol and centrifuged for 20 min at 14,000 rpm [26]. The experiment was carried out in vitro using ferric reducing antioxidant power (FRAP) to determine antioxidant capabilities. In this case, we used 0.25 mL of FRAP reagent, mixing FeCl 3 (20 mM) in acetate buffer (0.25 M, pH 3.6) at room temperature with 0.1 mL of diluted extract. For concentration calculation, calibration curve was performed using the standard Trolox (0.05-1 mM) as standard.

α-Amylase Inhibition Assay
The inhibition of pancreatic α-amylase inhibition was measured using Medicago sprout extract mixed with reaction solution starch (1 g/L) and phosphate buffer (pH 6.9). Then, 3 U/mL amylase enzyme was added to start the process [27]. After 10 min of incubation, 0.5 mL dinitro salicylic (DNS) reagent was added to terminate the reaction. The reaction mixture was heated to 100 • C for 10 min. Finally, the mixes received 0.5 mL of a 40 percent potassium sodium tartrate solution. At 540 nm, the absorbance was measured.

α-Glucosidase Inhibition Assay
The sprout hydroethanolic extract was combined with -glucosidase (2 U/mL) and incubated at 37 • C for 5 min to determine the inhibition of α-glucosidase [27]. After adding 1 mM para-nitrophenyl glucopyranoside dissolved in 50 mM phosphate buffer, the reaction buffer was incubated for 20 min at 37 • C (pH 6.8). A solution of sodium carbonate (1 M) was added to stop the process. The amount of para-nitrophenolate produced by para-nitrophenyl glucopyranoside was measured at 405 nm, and the inhibitory activity of -glucosidase was computed. The α-glucosidase inhibitory activity was expressed as percent inhibition and determined as follows: %inhibition = [(average A 405 control − average A 405 extractÞ/average A 405 control × 100].

Glycemic Index GI
The GI was determined using an in vitro starch hydrolysis method [27]. The process begins with the incubation of Medicago sprouts in a reaction buffer of HCl-KCl buffer (pH 1.5) for one hour at 40 • C under shaking conditions with pepsin (100 mg/mL). The mixture was then diluted in phosphate buffer (pH 6.9) before being incubated at 37 • C with α-amylase. 1 mL of aliquots were collected every 30 min and boiled for 20 min to cease the activity of the amylase enzyme. To convert the remaining starch to glucose, 0.4 M sodium acetate buffer (pH 4.75) and 60 L amyloglucosidase were added. For 50 min, the reaction mixture was incubated at 60 • C. Approximately 0.6 mL aliquots were collected and incubated at 37 • C for 35 min with 1.2 mL glucose oxidase/peroxidase. The mixture's absorbance was measured at 500 nm. The proportion of hydrolyzed starch at different times (0, 30, 60, 90, 120, and 180 min) was used to calculate the starch digestion rate. The area under the hydrolysis curve (AUC, 0-180 min) and hydrolysis were computed. The hydrolysis index was then computed by multiplying the difference between the AUC for a sample and the AUC for a standard by 100.

Statistical Analyses
The R statistics package was used to conduct the statistical analysis (Gplot, Agricola). All data were subjected to a one-way analysis of variance (ANOVA). As a post-hoc test for mean separations, Tukey's Test (p = 0.05) was used. Each experiment was repeated at least three times (n = 3). The R software created hierarchical clustering using Heatmap (Pearson correlation). The COrplot package was used to do correlation analysis on all of the data.

Growth and Photosynthetic Pigments of Medicago Sprouts
The fresh weight of sprouts showed a significant difference as a consequence of KNO 3 priming. As shown in Figure 1, the sprout primed with KNO 3 exhibited a significant increase in fresh weight (FW) in the three species, as compared to the control. Among the three species, the highest and most significant increase in FW was measured from Medicago interexta seeds priming with KNO 3 by 53%, while the FW of both Medicago indicus and Medicago polymorpha primed with KNO 3 increased only by 34% and 35%, respectively, as compared to control. In terms of the impact of KNO 3 priming on photosynthetic pigments, there was a clear rising trend in Medicago interexta sprout leaf pigments, which showed increases in chlorophyll a (Chla), chlorophyll b (Chlb), and total chlorophyll of 53%, 60%, and 56%, respectively, as compared to control ( Figure 1). Additionally, significant increases in Chla, Chlb, and total chlorophyll by 46%, 75%, and 56%, respectively, were recorded in Medicago polymorpha, as compared to control. Meanwhile, Medicago indicus sprouts showed an increase in chla by 38% and in total chlorophyll by 27%, while a slight increase was recorded in chlb. Furthermore, a significant amount of variation in carotenoid compounds in response to KNO 3 priming was associated with differences among Medicago species. Indeed, the highest increase of β-carotene, lutein, and Neoxanthin by 54% 58%, and 70% was recorded in Medicago interexta sprouts ( Figure 1). However, violaxanthin pigment was significantly increased in Medicago polymorpha and Medicago indicus by 36% and 35%, respectively, as compared to control.

Improvement of Nutritive Values: Mineral Content, Vitamins, and Antioxidant Activities
The Ca, K, Mg, Fe, Mn, and Zn concentrations, as well as Cu, were determined in dried Medicago sprouts. Regarding total nutrients analysis, the Ca, K, and Zn concentrations accounted for 24%, 22%, and 31%, respectively, on average in all species and treatment. However, Cu, Mg, Mn, and Fe were present in small amounts ( Table 1). The mineral content of sprouts is very dependent on the sprouting conditions and species. The KNO 3 priming increased the Ca, Cu, Fe, K, and P in the three species. Indeed, the greatest accumulation of K and P, by 2-and 5-fold, respectively, was observed in Medicago interexta sprouts. Likewise, KNO 3 priming increased the content of Zn in Medicago polymorpha and Medicago indicus by 36% and 21%, respectively, as compared to control, while no significant change was observed in Medicago interexta sprouts. Furthermore, Mn and Mg content increased by 36% and 37% in Medicago polymorpha, and by 50% and 26% in Medicago interexta. In contrast, the Mn and Mg were not affected by KNO 3 priming in Medicago indicus. An analysis of vitamins was carried out for three species of Medicago sprouts ( Table 2). The results revealed that Vit C presented the greatest accumulation by 41%, 32%, and 39% in Medicago indicus, Medicago polymorpha, and Medicago interexta, respectively (Table 1). KNO 3 priming enhanced the Vit C, Vit E, and riboflavin content in all three species. Obviously, Vit C content was higher in Medicago interexta in comparison to other species. Likewise, both Vit E and riboflavin showed the highest accumulation by 46% and 39%, respectively, in Medicago polymorpha compared to control and other species. In contrast, a slight increase in thiamine was recorded in Medicago indicus in a response to KNO 3 priming, and no significant change in Medicago polymorpha. While KNO 3 priming enhanced the thiamine content in Medicago interexta by 2-fold compared to control conditions.

Amino Acid Metabolism
HPLC analysis of amino acids in Medicago sprouts species revealed the presence of eighteen amino acids, with significantly different concentrations ( Table 3). The highest value was recorded for glutamine in Medicago interexta (2.17 mg/g dry wt), followed by asparagine, glycine, phenylalanine, serine, proline, threonine, isoleucine, valine, leucine, lysine, tryptophane, cysteine, histidine, alanine, methionine, arginine, and tyrosine. KNO 3 priming improved the accumulation of glutamine, serine, arginine, alanine, proline, histidine, valine, methionine, cystine, isoleucine, leucine, phenylalanine, tyrosine, lysine, threonine, and tryptophan in the three species. Indeed, the greatest accumulation was recorded in glutamine by 49% in Medicago interexta sprout. Likewise, Arginine showed the highest increase by 60% and 58% in Medicago indicus and Medicago polymorpha, respectively, compared to control. In contrast, the rest of amino acids were not significantly affected by KNO 3 priming, depending on Medicago species. Compared to control sprouts, the N content was significantly affected by KNO 3 in the three species. Unlike, the activities of nitrate reductase (NR), GDH, GOGAT, and GS were changed in response to KNO 3 priming, depending on species (Table 3). Indeed, the highest increase of NR, GDH, GOGAT, and GS, by 26%, 32%, 32%, and 19%, respectively, was recorded in Medicago interexta sprouts. Furthermore, the protein content decreased in Medicago indicus and Medicago polymorpha, whereas it increased by 13% in Medicago interexta, compared to control. Table 3. Effect of KNO 3 priming on total amino acids content, total N, proteins and NR, GDH and GOGAT activities of three species of Medicago sprouts, Values are represented by mean ± standard deviation of at least three independent replicates, Means marked by different letters are significantly different than control at p < 0.05.

Antioxidant Metabolites and Free Radical Scavenging Activity of Medicago Sprouts
The present results revealed that the priming with KNO 3 during germination has induced changes in phenolic compounds concentrations in Medicago sprouts ( Figure 2). KNO 3 priming significantly increased total phenolic and flavonoid contents in the three species.

Antioxidant Metabolites and Free Radical Scavenging Activity of Medicago Sprouts
The present results revealed that the priming with KNO3 during germination has induced changes in phenolic compounds concentrations in Medicago sprouts ( Figure 2). KNO3 priming significantly increased total phenolic and flavonoid contents in the three species. Besides, KNO3 priming enhanced the FRAP activities by 41%, 59%, and 35% for Medicago indicus, Medicago polymorpha, and Medicago interexta, respectively, in comparison to control (Figure 3). Furthermore, the reduced ascorbate and glutamine increased significantly (p < 0.05) in the three species as response to KNO3 priming, and the highest increase Besides, KNO 3 priming enhanced the FRAP activities by 41%, 59%, and 35% for Medicago indicus, Medicago polymorpha, and Medicago interexta, respectively, in comparison to control ( Figure 3). Furthermore, the reduced ascorbate and glutamine increased significantly (p < 0.05) in the three species as response to KNO 3 priming, and the highest increase was recorded in Medicago interexta (Figure 3).

Antidiabetic Activity
As shown in Figure 4, each species of Medicago sprouts exhibited antidiabetic activity. Under control conditions, Medicago interexta had the best inhibitory effect on α-amylase, while Medicago indicus had the best inhibitory effects on α-glucosidase. KNO 3 priming seemed to enhance the inhibition activity of α-amylase by 28% in Medicago indicus. Similarly, KNO 3 priming enhanced the inhibition activity of α-glucosidase by 30%, 40%, and 29% for Medicago indicus, Medicago polymorpha, and Medicago interexta, respectively, compared to control. The current results also demonstrated that KNO 3 priming caused a marked decrease in GI in Medicago polymorpha and Medicago interexta (lower than 70).

Principal Component Analysis (PCA)
PCA is a multivariate statistical analysis that can be used to examine and simplify complex and huge datasets. The pattern of variation in Medicago species was also analyzed

Principal Component Analysis (PCA)
PCA is a multivariate statistical analysis that can be used to examine and simplify complex and huge datasets. The pattern of variation in Medicago species was also analyzed using principal component analysis (PCA) to evaluate the variety of the species and their link with the observed traits based on the correlation between the traits and extracted clusters. The chemical profiles of plants that were not primed with KNO 3 were grouped and clearly separated from sprouts primed with KNO 3 . In our dataset, two groups of traits were identified in the PCA biplot considering both PC1 and PC2 simultaneously (Figures 5 and 6). The FW, leaf pigments, mineral content, N metabolism, polyphenols, antioxidants enzymes, and glucosidase and amylase inhibitor enzymes linked with Medicago interexta and polymorpha primed with KNO 3 .

KNO3 Priming Increased Biomass Accumulation in Medicago Sprouts
Seed priming is used to ensure rapid and uniform seed germination and seedling emergence in order to improve agricultural production performance. Priming with KNO3 has also been found to boost seedling germination, growth, establishment, and productivity in numerous studies. Seed priming has been extensively studied in terms of plant ecology, physiology, cellular biology, and molecular biology [28,29]. Increased seed quality has recently become a top focus in the agriculture business. Seed priming with KNO3 increased the growth of three Medicago species in the current study. The results were similar to those of earlier studies, which reported that KNO3 priming enhanced cucumber [30], white clover [31], and soybean [32] seedling fresh weights, when compared with unprimed seedlings. Similarly, seeds of Medicago sativa var. Anand-z primed with 0.1 percent MgCl2 also had a high rate of seed germination and seedling growth [33]. Enhancement of Medicago growth might be due to increased cell division and elongation and activation of ROS scavenging enzymes in KNO3 primed seeds [30]. KNO3 may promote the growth of Medicago sprouts by acting as nutrients and initiators of crucial emergence and growth processes in sprouts. The improvement of growth by KNO3 priming seemed to be varied among the species of Medicago. Indeed, Medicago interexta presented the highest biomass accumulation compared to other species. Differences in emergence and growth among species in response to germination conditions were reported in several research works [34]. The results could be confirmed by the photosynthetic pigments contents of Medicago sprouts, where the contents of chla, chlb, and total chlorophyll were generally significantly increased in response to KNO3 priming sprouts. Furthermore, the enhancement of chlorophyll biosynthesis by KNO3 was inconsistent with the increases of Mg 2+ contents in Medicago polymorpha and Medicago interexta. The chlorophyll molecule containing Mg covalently linked with four nitrogen (N) atoms, and this might be the reason that KNO3

KNO 3 Priming Increased Biomass Accumulation in Medicago Sprouts
Seed priming is used to ensure rapid and uniform seed germination and seedling emergence in order to improve agricultural production performance. Priming with KNO 3 has also been found to boost seedling germination, growth, establishment, and productivity in numerous studies. Seed priming has been extensively studied in terms of plant ecology, physiology, cellular biology, and molecular biology [28,29]. Increased seed quality has recently become a top focus in the agriculture business. Seed priming with KNO 3 increased the growth of three Medicago species in the current study. The results were similar to those of earlier studies, which reported that KNO 3 priming enhanced cucumber [30], white clover [31], and soybean [32] seedling fresh weights, when compared with unprimed seedlings. Similarly, seeds of Medicago sativa var. Anand-z primed with 0.1 percent MgCl 2 also had a high rate of seed germination and seedling growth [33]. Enhancement of Medicago growth might be due to increased cell division and elongation and activation of ROS scavenging enzymes in KNO 3 primed seeds [30]. KNO 3 may promote the growth of Medicago sprouts by acting as nutrients and initiators of crucial emergence and growth processes in sprouts. The improvement of growth by KNO 3 priming seemed to be varied among the species of Medicago. Indeed, Medicago interexta presented the highest biomass accumulation compared to other species. Differences in emergence and growth among species in response to germination conditions were reported in several research works [34]. The results could be confirmed by the photosynthetic pigments contents of Medicago sprouts, where the contents of chla, chlb, and total chlorophyll were generally significantly increased in response to KNO 3 priming sprouts. Furthermore, the enhancement of chlorophyll biosynthesis by KNO 3 was inconsistent with the increases of Mg 2+ contents in Medicago polymorpha and Medicago interexta. The chlorophyll molecule containing Mg covalently linked with four nitrogen (N) atoms, and this might be the reason that KNO 3 priming enhanced nutrients uptake and resulted to enhanced chlorophyll contents in Medicago sprouts leaves. The results are in agreement with previous studies, which reported that biopriming significantly enhanced chlorophyll contents in wheat leaves [35]. Furthermore, many works reported that lucerne possesses detoxifying and anticancerogenic properties due to its high chlorophyll content [35]; thus, it seemed that KNO 3 priming could enhanced these proprieties in the three species. Moreover, the results revealed that the KNO 3 priming enhanced the two groups of carotenoids, including β-carotene and hydroxylated carotenoids, designated as xanthophyll pigments, such as lutein, neoxanthin, and violaxanthin. Many reports revealed that Medicago contains 400-500 mg total carotenoids/kg, with the majority being xanthophylls, such as lutein and zeaxanthin [36]. Furthermore, a review of xanthophylls' possible functions in disease prevention has revealed that they may have a preventive impact against some malignancies, coronary heart disease, and stroke. Besides, lutein, neoxanthin, and violaxanthin pigments possess anti-inflammatory and strong antioxidant properties, and they are very active against liver neoplasms [37].

KNO 3 Priming Increases Nutritive Values of Medicago Sprouts
Mineral and vitamin deficiencies have been linked to a variety of detrimental health impacts in humans. Sprouts have long been thought to be a good source of bioavailable minerals, such as Fe, Zn, Mn, Mg, Cu, and Ca [38]. As a result, using KNO 3 priming to increase the mineral element content of sprouts could improve the nutritional and healthpromoting effects of Medicago sprouts. In the present study, KNO 3 priming resulted in a significant increment in minerals nutrition concentration (Ca, Cu, Fe, Mn, K, and P) in the three species. The mineral content of sprouts is highly dependent on the sprouting conditions in general; however, the mineral contents observed in the sprouts analyzed in this study are consistent with those described in the literature [1]. Supporting our results, KNO 3 priming enhanced leaf nutrient accumulation and significantly enhanced seedling growth in mung beans [29] and cucumber seedlings [30]. Furthermore, the increase in mineral content varied between species. Medicago interexta presented the highest increment in Ca content. The high content of Ca makes these products suitable for consumers with lactose intolerance [39]. Other minerals, such as Fe, were also quantified in Medicago interexta, being higher than the ones reported for other species. The high content of Fe could be helpful to prevent anemia caused by iron deficiency [39].
Concerning vitamins, this outcome revealed that the Medicago sprouts were rich in Vit E (tocopherol), and its content varied between species, since Medicago polymorpha and Medicago interexta showed the greatest levels. Besides, KNO 3 priming enhanced the accumulation of Vit E and riboflavin in the three species, but it decreased the level of thiamine in Medicago polymorpha. The positive effect of KNO 3 priming on vitamins content makes Medicago species a remarkable source of vitamins for supporting immunity.

KNO 3 Priming Promotes N assimilation in Medicago Sprouts
It is widely recognized that the essential amino acid content in plants is well acknowledged to have a substantial impact on their nutritional and health-promoting characteristics. Essential amino acids are critical for human health since they cannot be generated from scratch and act as building blocks for a variety of proteins that play critical roles in human health [40]. For instance, lucerne was approved for use in human nutrition [41]. The outcomes of the present study revealed that Medicago sprouts were rich in essential and semi-essential amino acids, such as glutamine, phenylalanine, threonine, asparagine, and glycine, which are considered as the most important bioactive components. Further, KNO 3 priming enhanced the accumulation of proline, histidine, valine methionine cystine, and isoleucine. Moreover, the effect of KNO 3 priming varied between the three species, since some amino acids greatly increased Medicago polymorpha and Medicago interexta more than Medicago indicus. In line with our findings, a previous study discovered that the response of plants to environmental conditions in primary N absorption differed by species [13]. The amino acid in Medicago sprouts is present in substantially larger concentrations than in eggs or wheat and was approved for use in human nutrition [41]. This increment in several amino acids in response to KNO 3 priming has resulted in increases in total N in the three species and total protein in Medicago interexta. The increase in the activity of important enzymes in N metabolism, including NR, GS, GDH, and GOGAT, could explain the changes in amino acid levels. We suggested that the nitrate supplemented by the priming with KNO 3 had a positive effect on NR. In fact, the increases in the activity of nitrate reductase (NR) increased the potential for nitrate reduction, resulting in increased capacity for amino acid synthesis, protein synthesis, and total N assimilation [12]. These results were in accordance with the results obtained in leaves of wheat seedlings [12] and Safflower [42] treated with KNO 3 . Concerning the total protein, the increase in this compound in response to KNO 3 priming, except in Medicago interexta, may be due to the direct involvement of K in several steps of the translocation process, including the binding of RANt to ribosomes [13]. Interestingly, here, the KNO 3 priming effect on N level and GS, GDH, and GOGAT enzymes activities were varied with different species.

Antioxidant Metabolites Accumulation Increased Antioxidant Biological Activity of Medicago Sprouts Extracts
The bioactive compounds of Medicago have gotten a lot of interest because of their antibacterial, anti-inflammatory, anticancer, and antioxidant properties [7]. These biological actions, which include anti-inflammatory and antioxidant properties, may be due to the presence of phenolic and flavonoids chemicals, which function as free radical scavengers and/or metal chelators [43]. Caunii et al. (2012) [44] found that the lucerne extract included a number of free hydroxyl groups (hydrogen donors), giving the product a significant antioxidizing effect in the human body. As such, the outcomes of the current study revealed that KNO 3 enhanced the antioxidants properties of Medicago sprouts, and the increases depend on species. Indeed, Medicago polymorpha exhibit the highest antioxidant activities since flavonoids reduced glutathion and ascorbate content, and FRAP showed an increment by 2-fold, compared to control. This suggests that the obtained values of these compounds are impacted by species and germination processes.
As antidiabetic agents, the leaves of Medicago have been used traditionally to reduce plasma glucose levels in diabetic subjects [45,46]. In this investigation, the accumulation of nitrogen compounds enhanced by KNO 3 priming increased the antidiabetic activity of Medicago sprouts extracts, since the GI decrease sharply mainly in Medicago interexta compared to others sprouts in response to KNO 3 priming. Furthermore, the current study illustrated that KNO 3 priming enhanced the inhibitor effect against α-amylase and α-glucosidase in the three species of Medicago sprouts. Following the previous studies and examination, the anti-diabetic activity of Medicago was tested against α-amylase [46]. The accumulation of N leads to an increase in amino acid synthesis. Hence, amino acids may regulate insulin secretion in several ways, including the production of metabolic coupling factors, plasma membrane depolarization, and mitochondrial function augmentation [40]. Furthermore, the enhancement in several enzymes of N metabolism caused a high production of glutamine. This former amino acid has been postulated to play a role in nutrient-induced stimulus-secretion coupling as an additive factor in the glucose-stimulated insulin secretion amplification pathway [40]. Overall, as antidiabetic agents, accumulation of nitrogenous compounds can explain the increased antidiabetic activity of Medicago sprouts extracts.

Species-Specific Responses to KNO 3 Priming
According to hierarchical clustering, the effect of KNO 3 seemed to be related to Medicago species (Figure 3). The genetic diversity of Medicago has been identified by numerous studies [47]. Besides, Medicago was considered as the genetically complex species [48]. These findings indicate that there is a genotypic difference in seed priming efficacy, which is in accordance with other studies [47,48]. The differences between the three species may be due to ontogeny and species diversity. Medicago indicus sprouts primed by KNO 3 showed the highest antioxidant and antidiabetics activities. Besides, it seemed that KNO 3 improved the nutritive value of these farmer sprouts by enhancing the accumulation of vitamins (Vit E and Vit C), proteins, mineral nutrients, and nitrogen, followed by Medicago interexta and Medicago polymorpha, which responded to KNO 3 priming by enhancing the accumulation of the major amino acids.

Conclusions
The use of KNO 3 priming to improve the biological and nutritional qualities of Medicago sprouts has been proven to be effective. Hence, Medicago sprouts are increasingly being used as an alternative source of natural antioxidant and mineral components in ready-to-eat fresh products or the manufacture of new safe functional foods. At the species level, Medicago interexta and Medicago polymorpha were more responsive to the KNO 3 positive effect, being better than other species (Medicago indicus), since it gave the highest antioxidant and antidiabetic activities.